WO1987005624A1 - Biochemical detector - Google Patents

Biochemical detector Download PDF

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Publication number
WO1987005624A1
WO1987005624A1 PCT/GB1987/000192 GB8700192W WO8705624A1 WO 1987005624 A1 WO1987005624 A1 WO 1987005624A1 GB 8700192 W GB8700192 W GB 8700192W WO 8705624 A1 WO8705624 A1 WO 8705624A1
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WIPO (PCT)
Prior art keywords
enzyme
analyte
polymer
hydrogen peroxide
support element
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Application number
PCT/GB1987/000192
Other languages
French (fr)
Inventor
Colin James Suckling
Richard Arthur Pethrick
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University Of Strathclyde
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
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Publication date
Application filed by University Of Strathclyde filed Critical University Of Strathclyde
Priority to AT87901601T priority Critical patent/ATE76097T1/en
Priority to DE8787901601T priority patent/DE3779036D1/en
Publication of WO1987005624A1 publication Critical patent/WO1987005624A1/en

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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M41/00Means for regulation, monitoring, measurement or control, e.g. flow regulation
    • C12M41/30Means for regulation, monitoring, measurement or control, e.g. flow regulation of concentration
    • C12M41/32Means for regulation, monitoring, measurement or control, e.g. flow regulation of concentration of substances in solution
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/001Enzyme electrodes
    • C12Q1/005Enzyme electrodes involving specific analytes or enzymes

Definitions

  • the present invention relates to a device for use in the detection of biochemical analytes in liquid samples.
  • the present invention provides a device for use in the detection, in a liquid sample, a predetermined analyte which is reactive under predetermined enzyme catalysed conditions so as to release at least one of a proton and hydrogen peroxide, which device comprises an electrically conducting polymer element having spaced apart connection means for connection of said polymer element, in use of the device, to an electrical circuit means for directly or indirectly detecting changes in electrical resistance in said element, said polymer containing conjugatable monomer units and being permeable to protons and where said analyte under said enzyme catalyzed conditions produces hydrogen peroxide, to hydrogen peroxide and having an electrical conductivity which is variable according to the amount of protons or hydrogen peroxide in contact therewith, and an enzyme support element containing at least one enzyme and any cofactor(s) required in said predetermined enzyme-catalyzed conditions, in an analyte permeable substantially non-conducting medium and having a first face in contact with said polymer element and a second face disposable, in use, directly or
  • the device includes a filter means selectively permeable to the analyte which filter means is disposed at said second face for screening said enzyme support element from at least one other component, most preferably substantially all other components, of said liquid sample in use of the device.
  • the polymer is reduced prior to immersion in the unknown analyte containing solution in order to increase the sensitivity of the device.
  • Reduction may be effected by any suitable means but conveniently is effected by immersion in an aqueous alkaline solution such as dilute sodium hydroxide.
  • the amount of analyte present is obtained as a change in electrical conductivity which can be simply measured by connnecting to said connection means any of a variety of readily available and/or relatively inexpensive means such as an ohm meter or resistance bridge circuit. It may moreover be noted that unlike certain previous systems, the device of the present invention does not in general require the use of any special environmental operating conditions such as anaerobic conditions.
  • the device may be made in various shapes and sizes but will generally be in the form of a multilayer thin film device made up of a thin film polymer element coated on one or both sides with the enzyme support element. Where only one side is coated with the support element then the other side will normally be sealed with an impermeable coating to avoid extraneous interactions with the polymer element. Where a filter means is provided this will generally be in the form of a further coating on top of the enzyme support element coating.
  • connection means are normally in the form of highly conductive metal electrodes e.g. of platinum, silver, gold or copper, extending into the polymer element. Conveniently these electrodes can be used as a support for the polymer element, the latter being in the form of a film coating encasing part of the electrodes.
  • Suitable polymers will in general have a conductivity in the range from 10 -4 to 102S cm-1
  • polymers that may be mentioned include polypyrrole and polymers based on aniline and pyridine or other quaternisable conjugated monomer units.
  • polymers In the case of devices using enzyme systems producing protons the polymer should have protonatable monomer units containing quaternisable nitrogen atoms - as for example in the specific examples mentioned in the preceding sentence.
  • the polymers may be prepared by any suitable method known in the art for the production of these materials in a suitable form with the desired conductivity.
  • the polymer may be made by electrochemical polymerisation in an electrochemical cell containing a solution of the monomer, together with a suitable amount of an electrical conductivity promoting dopant, in an electrochemically stable relatively polar solvent capable of maintaining ionic species in solution therein and thereby maintaining the conductivity of the solution in said electrochemical cell.
  • Suitable dopants are known in the art including strong protonic acids such as for example sulphonic acids, perchloric acid, and fluoroboric acid.
  • the dopants may be employed in various proportions in the polymer especially in relation to conductivity, stability, and/or tractability as well as the nature of the individual dopant.
  • the - dopant is used in a molar ratio of from 4 to 2 : 1 relative to the polymer repeating unit, preferably from 4 to 3 : 1.
  • an electrochemical cell having two electrodes, usually of highly conductive metal such as platinum, gold, or silver, across which is applied a voltage in the range from 0.5V above to 0.5V below the oxidation - reduction potential of the polymer.
  • a reference electrode e.g.
  • a standard calomel electrode is included in the cell to facilitate monitoring and control of the voltage at the electrode at which the polymer is formed to within the desired range.
  • SCE standard calomel electrode
  • the electrode at which the polymer is formed is generally maintained at a voltage of 0.5V to 1.5V relative to the SCE.
  • the elctrochemical polymerisation conditions such as applied voltage, temperature, solvent, monomer and dopant concentrations, rate of polymerisation, and electrode configuration may be varied to a greater or lesser extent to facilitate production of the polymer in a suitable form which will generally be a thin film.
  • Suitable polymer, especially polypyrrole, thin films are commercially available, e.g. from the Polaroid Corporation of Cambridge, Mass., U.S.A.
  • soluble polymers which are soluble in organic solvents such as acetonitrile and dimethyl ⁇ formamide, the polymer can be initially produced in a different form e.g.
  • a suitable substrate e.g. a printed circuit board or the like having conductor tracks thereon formed and arranged to provide the electrical connections from the polymer to a suitable resistance measuring means which may if desired also be mounted on said printed circuit board or the like.
  • the electrochemical polymerisation conditions may also be varied to adjust the conductivity of the polymer.
  • the polymer should desirably have a conductivity in the range from 10 -4 to 102S cm-1 depending upon such factors as the sensitivity of the resistance measuring means to be used with the device and the analyte concentration range to be measured. Further details of suitable processes for the preparation of conductive polymers are disclosed in for example F.M.Al-Arrayed et al in Materials Forum, 1986, 9_, 209-216.
  • Various direct or indirect resistance/conductivity measuring means may be used to monitor the changes in conductivity of the polymer when the device is contacted with an analyte containing solution.
  • a standard ohm meter or resistance bridge device for measuring the resistance of the device and formed and arranged for indicating the absolute value of the resistance.
  • a measuring means formed and arranged to display or otherwise output data indicating directly analyte concentrations corresponding to the changes in conductivity occurring. It will be appreciated that the conductivity of some polymer film preparations is time dependent.
  • the rate of response of the device of the invention in terms of establishing equilibrium conditions throughout the polymer element will vary significantly with inter alia the configuration of the polymer element and its surface area in contact with the enzyme support element, relative to the volume of said polymer element. Accordingly in use of the device it may be necessary on the one hand to measure the initial conductivity before the device is introduced to the analyte containing solution and at a suitable time after contact with the analyte containing solution to determine the relative change in conductivity, and on the other hand to monitor variation of conductivity over a period of time following initial exposure. In such cases the device would advantageously be used with suitable data recording and/or data processing means adapted to correlate the differences and/or variations in conductivity to analyte concentration in accordance with previously established relationships based on determinations of known analyte solutions.
  • Suitable system for the determination of alcohol analytes uses an alcohol dehydrogenase to catalyse oxidation of the alcohol e.g. ethanol to acetaldehyde, by NAD with the liberation of protons.
  • a system suitable for the determination of lactic acid uses lactate dehydrogenase to catalyse oxidation of the lactic acid to pyruvic acid by NAD.
  • Another system using steroid dehydrogenases and NAD can also be used to determine certain steroids.
  • Another system which is suitable for glutamic acid determination uses glutamate dehydrogenase to catalyse oxidation of the glutamic acid to 2-oxoglutamic acid by NAD with the liberation of protons.
  • An enzyme system suitable for the determination of glucose comprises glucose oxidase which catalyses oxidation of glucose to gluconic acid with the liberation of hydrogen peroxide.
  • Another system of this type can be used to determine cholesterol using the enzyme cholesterol oxidase again with the liberation of hydrogen peroxide.
  • Certain amines and amino acids can be similarly detected using the appropriate amine or amino acid oxidase.
  • analytes may be detected through the use of enzymes linked to antibodies to said analytes so that binding of the analyte with the antibody converts the enzyme from a catalytically inactive form to a catalytically active form which can then catalyse release of protons or hydrogen peroxide by a suitable reactant.
  • analytes such as cytotoxic drugs e.g. ethotrexate; food toxins e.g. aflatoxins which are produced by moulds growing on peanuts, maize and wheat; and industrial effluents and toxic products, e.g. dioxin, may be determined using devices of the invention.
  • a suitable enzyme which catalyzes release of protons or hydrogen peroxide by suitable reagents is conjugated to a sample of the desired analyte, by means of suitable protein modifying reactions e.g. using a carbodiimide to produce linking of carboxyl and amino groups, using reductive amination of aldehydes using sodiumcyanoborohydride and an amine; using acylation of amino groups with anhydrides; or any other suitable procedure known in the art.
  • suitable protein modifying reactions e.g. using a carbodiimide to produce linking of carboxyl and amino groups, using reductive amination of aldehydes using sodiumcyanoborohydride and an amine; using acylation of amino groups with anhydrides; or any other suitable procedure known in the art.
  • suitable protein modifying reactions e.g. using a carbodiimide to produce linking of carboxyl and amino groups, using reductive amination of aldehydes using sodiumcyanoborohydride and an amine;
  • the enzyme support element is advantageously coated with a filter means for screening said enzyme support element and the polymer element to a greater or lesser extent from other materials present in the liquid sample to be tested which could interact with one or more of the enzyme, the enzyme catalysed reaction, and the polymer element.
  • a filter means for screening said enzyme support element and the polymer element to a greater or lesser extent from other materials present in the liquid sample to be tested which could interact with one or more of the enzyme, the enzyme catalysed reaction, and the polymer element.
  • the liquid sample is a biological fluid such as urine or a blood fraction which contains a whole variety of different substances.
  • the filter means used will be substantailly impermeable to proteinaceous material and/or macromolecular substances.
  • Suitable filter means include highly crosslinked polymeric water- swellable gels such as polyacrylamide and polysaccharose gels.
  • the filter means is conveniently in the form of a layer secured to the outer face of the conducting polymer film for example by polymerisation thereon in the case of a polymeric gel or by mechanical securing with the aid of external mechanical supports or restraints.
  • the device may conveniently be mounted in a housing of an inert and impermeable electrically insulating material e.g. a plastics material such as polyvinylchloride, with a 'window' opening across a central area of the outer face of the filter means.
  • the present invention provides a method of detecting a predetermined analyte in a liquid sample comprising the steps of contacting the liquid sample with the second face of the enzyme support element of the device of the invention either directly or through a filter means, selectively permeable to the analyte, and measuring the change in resistance between the connection means of the polymer element of said device.
  • Fig. 1 is a generally schematic sectional elevation of a device of the invention in use in measuring the ethanol content of a liquid sample L.
  • Fig. 1 shows a device of the invention comprising a vessel 1 of an inert electrically insulating material such as glass having an electrically conducting polypyrrole layer 2 in the bottom 3 thereof.
  • An ethanol permeable substantially electrically non-conducting enzyme support layer 4 is disposed on top of said polypyrrole layer 2 with a first face 5 in contact with the latter and a second face 6 covered in turn by a filter means layer 7.
  • Two spaced apart electrical connections in the form of platinum wires 9 extend through the bottom wall 10 of the vessel 1 into the polypyrrole layer 2 and are connected 12 at their distal ends 13 to an ohm meter_ £_.
  • the enzyme support layer comprises a highly cross- linked polymeric water-swellable gel such as a polyacrylamide or polysaccharose gel to which is secured the enzyme(s) to be used together with any necessary cofactors.
  • a highly cross- linked polymeric water-swellable gel such as a polyacrylamide or polysaccharose gel to which is secured the enzyme(s) to be used together with any necessary cofactors.
  • a prepolymer of polyacrylamide having a molecular weight in the range from 1000 to 2000 to which is added ethanol dehydrogenase, and the co-enzymes NAD.
  • the prepolymer is then cross-linked in conventional manner to entrap the enzyme and co-enzyme.
  • a data processing unit D is connected thereto.
  • This unit is adapted to record differences in resistance measurements between successive readings and process these in accordancewith previously established relationships obtainedusing known solutions to provide an output signal corresponding to the ethanol concentration present which is then displayed on a suitable visual display unit E>.
  • EXAMPLE 1 Construction of Ethanol Sensor Polypyrrole Film (2.5 x 1.1 cms. 0.2mm thick) was mounted on a glass slide support using two metal conductor legs secured to the film in spaced apart relation, with the aidof a suitable non-conducting resin adhesive such as that available under the Trade Name "Araldite” from the Ciba-Geigy Company of Basel Switzerland.
  • This resin was also used to provide an insulating coating for the legs between the slide and the film. Suitable conductor leads for attachment to a conductivity orohm meter were connected to the metal conductor legs on the slide. The film element was then placed in a vessel to which was added activated polyacrylamide prepolymer (PAN)
  • the Ethanol Sensor of Example I was first deprotonated by immersion in aqueous sodium hydroxide (1M) for 5 minutes. (If desired lower concentrations e.g. 0.5M can be used provided the immersion time is extended appropriately - to 30 minutes in this case.)
  • the Ethanol Sensor was then equilibrated by immersion in deionised water, removed from the water, superficial water shaken off, and the conductivity of the sensor then determined using a Solartron Schlumberger 1186 Electrochemical interface (available from the Solartron Limited of Farnborough, Hampshire, England). Ethanol (100 ⁇ l) was added to deionised water to give an ethanol concentration of 10 mM and the sensor immersed in the solution. The procedure formeasuring conductivity was repeated after successfive periods of 2 minutes immersion. Results
  • the glucose Sensor was equilibrated by immersion in deionised water, the superficial water shaken off, and the conductivity determined as described in Example III.
  • Glucose 100 mg was added to give a solution concentration of 30 mM and the sensor immersed in the solution.
  • the procedure for determining conductivity was repeated after successive periods of 2 minutes immersion. Results After 4 minutes, the current increase was 30 mA and reached a maximumof40 mA in 20 minutes. Following the same procedures but using two slightly thinner films prepared independently under substantially identical conditions a test solution containing 25mM glucose yielded current increases after 20 minutes of 37ma and 40 a .
  • EXAMPLE V Preparation of cholesterol sensor The procedure in Example I for the preparation of an ethanol sensor was followed except that cholesterol oxidase (1 mg, Sigma Chemical Co. Ltd., Poole, England) replaced alcohol dehydrogenase and nicotinamide adenine dinucleotide. The gelling time was 2% in and cross- linking time was 2 minutes.
  • EXAMPLE VI Detection of cholesterol The cholesterol sensor was equilibrated as in Example III for the detection of ethanol. Its response to solutions of cholesterol water-containing 10% Brij 30 (a non-ionic polyethyleneoxide detergent available from I.C.I, pic of England)was determined. Results

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Abstract

A device for use in the detection, in a liquid sample, of a predetermined analyte which is reactive under predetermined enzyme catalysed conditions so as to produce at least one of a proton and hydrogen peroxide. The device comprises an electrically conducting polymer element (2) having spaced apart connections (9) to an electrical circuit means (12) for directly or indirectly detecting changes in electrical resistance in the element (2). The polymer (2) contains conjugatable monomer units and is permeable to protons and where said analyte under said enzyme catalyzed conditions produces hydrogen peroxide, to hydrogen peroxide. The polymer (2) further has an electrical conductivity which is variable according to the amount of protons or hydrogen peroxide in contact therewith, and an enzyme support element (4) containing at least one enzyme and any cofactor(s) required in the predetermined enzyme-catalysed conditions, in an analyte permeable substantially non-conducting medium and also has a first face (5) in contact with the polymer element (2) and a second face (6) disposable in contact with the liquid sample. The present invention also provides a method of detecting a predetermined analyte in a liquid sample comprising the steps of contacting the liquid sample with the second face (6) of the enzyme support element (4) of the device and measuring the change in resistance between the connection means (9).

Description

BIOCHEMICAL DETECTOR
The present invention relates to a device for use in the detection of biochemical analytes in liquid samples.
The regular monitoring of various biochemical analyte levels in body fluids is extremely important in the management of certain conditions as for example in the case of diabetes where various methods have been previously proposed for measuring glucose levels in solutions thereof. In one such method an enzyme catalysed reaction of glucose is monitored via changes in fluorescence spectra resulting from the reaction. In another method an oxygen electrode is provided with a glucose oxidase enzyme coating and the reduction in the level of oxygen reaching the electrode due to consumption thereof by an, enzyme catalysed reaction of glucose with oxygen in said coating is used to obtain an indication of the amount of oxygen reaching the electrode. In both cases it will be noted that the methods employed involve the use of relatively cumbersome and/or specialized and expensive apparatus thereby limiting the circumstances under which glucose determinations can be carried out.
It is an object of the present invention to avoid or minimize one or more of the above disadvantages.
The present invention provides a device for use in the detection, in a liquid sample, a predetermined analyte which is reactive under predetermined enzyme catalysed conditions so as to release at least one of a proton and hydrogen peroxide, which device comprises an electrically conducting polymer element having spaced apart connection means for connection of said polymer element, in use of the device, to an electrical circuit means for directly or indirectly detecting changes in electrical resistance in said element, said polymer containing conjugatable monomer units and being permeable to protons and where said analyte under said enzyme catalyzed conditions produces hydrogen peroxide, to hydrogen peroxide and having an electrical conductivity which is variable according to the amount of protons or hydrogen peroxide in contact therewith, and an enzyme support element containing at least one enzyme and any cofactor(s) required in said predetermined enzyme-catalyzed conditions, in an analyte permeable substantially non-conducting medium and having a first face in contact with said polymer element and a second face disposable, in use, directly or indirectly in contact with a said liquid sample.
Preferably the device includes a filter means selectively permeable to the analyte which filter means is disposed at said second face for screening said enzyme support element from at least one other component, most preferably substantially all other components, of said liquid sample in use of the device.
Desirably in the case of a device of the invention based on the production and detection of protons, the polymer is reduced prior to immersion in the unknown analyte containing solution in order to increase the sensitivity of the device. Reduction may be effected by any suitable means but conveniently is effected by immersion in an aqueous alkaline solution such as dilute sodium hydroxide.
With a device of the present invention the amount of analyte present is obtained as a change in electrical conductivity which can be simply measured by connnecting to said connection means any of a variety of readily available and/or relatively inexpensive means such as an ohm meter or resistance bridge circuit. It may moreover be noted that unlike certain previous systems, the device of the present invention does not in general require the use of any special environmental operating conditions such as anaerobic conditions.
The device may be made in various shapes and sizes but will generally be in the form of a multilayer thin film device made up of a thin film polymer element coated on one or both sides with the enzyme support element. Where only one side is coated with the support element then the other side will normally be sealed with an impermeable coating to avoid extraneous interactions with the polymer element. Where a filter means is provided this will generally be in the form of a further coating on top of the enzyme support element coating.
The connection means are normally in the form of highly conductive metal electrodes e.g. of platinum, silver, gold or copper, extending into the polymer element. Conveniently these electrodes can be used as a support for the polymer element, the latter being in the form of a film coating encasing part of the electrodes.
Various electrically conducting polymers containing conjugated monomer units may be used for the polymer element. Suitable polymers will in general have a conductivity in the range from 10 -4 to 102S cm-1
Particular polymers that may be mentioned include polypyrrole and polymers based on aniline and pyridine or other quaternisable conjugated monomer units. In the case of devices using enzyme systems producing protons the polymer should have protonatable monomer units containing quaternisable nitrogen atoms - as for example in the specific examples mentioned in the preceding sentence.
The polymers may be prepared by any suitable method known in the art for the production of these materials in a suitable form with the desired conductivity. In general though the polymer may be made by electrochemical polymerisation in an electrochemical cell containing a solution of the monomer, together with a suitable amount of an electrical conductivity promoting dopant, in an electrochemically stable relatively polar solvent capable of maintaining ionic species in solution therein and thereby maintaining the conductivity of the solution in said electrochemical cell. Various suitable dopants are known in the art including strong protonic acids such as for example sulphonic acids, perchloric acid, and fluoroboric acid. The dopants may be employed in various proportions in the polymer especially in relation to conductivity, stability, and/or tractability as well as the nature of the individual dopant. Usually though the - dopant is used in a molar ratio of from 4 to 2 : 1 relative to the polymer repeating unit, preferably from 4 to 3 : 1. In general there is used an electrochemical cell having two electrodes, usually of highly conductive metal such as platinum, gold, or silver, across which is applied a voltage in the range from 0.5V above to 0.5V below the oxidation - reduction potential of the polymer. In practice a reference electrode e.g. a standard calomel electrode (SCE) is included in the cell to facilitate monitoring and control of the voltage at the electrode at which the polymer is formed to within the desired range. Where an SCE reference electrode is used the electrode at which the polymer is formed is generally maintained at a voltage of 0.5V to 1.5V relative to the SCE.
It will be appreciated that the elctrochemical polymerisation conditions such as applied voltage, temperature, solvent, monomer and dopant concentrations, rate of polymerisation, and electrode configuration may be varied to a greater or lesser extent to facilitate production of the polymer in a suitable form which will generally be a thin film. Suitable polymer, especially polypyrrole, thin films are commercially available, e.g. from the Polaroid Corporation of Cambridge, Mass., U.S.A. In the case though of soluble polymers which are soluble in organic solvents such as acetonitrile and dimethyl¬ formamide, the polymer can be initially produced in a different form e.g. a granular form where this is more convenient and then dissolved in a suitable solvent to form a solution which can be applied to a suitable substrate e.g. a printed circuit board or the like having conductor tracks thereon formed and arranged to provide the electrical connections from the polymer to a suitable resistance measuring means which may if desired also be mounted on said printed circuit board or the like.
The electrochemical polymerisation conditions may also be varied to adjust the conductivity of the polymer. In general the polymer should desirably have a conductivity in the range from 10 -4 to 102S cm-1 depending upon such factors as the sensitivity of the resistance measuring means to be used with the device and the analyte concentration range to be measured. Further details of suitable processes for the preparation of conductive polymers are disclosed in for example F.M.Al-Arrayed et al in Materials Forum, 1986, 9_, 209-216.
Various direct or indirect resistance/conductivity measuring means may be used to monitor the changes in conductivity of the polymer when the device is contacted with an analyte containing solution. Thus for example there could be used a standard ohm meter or resistance bridge device for measuring the resistance of the device and formed and arranged for indicating the absolute value of the resistance. In general though it will be more convenient to use a measuring means formed and arranged to display or otherwise output data indicating directly analyte concentrations corresponding to the changes in conductivity occurring. It will be appreciated that the conductivity of some polymer film preparations is time dependent. Also the rate of response of the device of the invention in terms of establishing equilibrium conditions throughout the polymer element will vary significantly with inter alia the configuration of the polymer element and its surface area in contact with the enzyme support element, relative to the volume of said polymer element. Accordingly in use of the device it may be necessary on the one hand to measure the initial conductivity before the device is introduced to the analyte containing solution and at a suitable time after contact with the analyte containing solution to determine the relative change in conductivity, and on the other hand to monitor variation of conductivity over a period of time following initial exposure. In such cases the device would advantageously be used with suitable data recording and/or data processing means adapted to correlate the differences and/or variations in conductivity to analyte concentration in accordance with previously established relationships based on determinations of known analyte solutions.
Various enzyme catalyzed reaction systems are known in the art which generate protons or hydrogen peroxide in enzyme catalyzed reactions of analytes either directly or with derivatives obtained by further enzyme catalysed reactions. One suitable system for the determination of alcohol analytes uses an alcohol dehydrogenase to catalyse oxidation of the alcohol e.g. ethanol to acetaldehyde, by NAD with the liberation of protons. A system suitable for the determination of lactic acid uses lactate dehydrogenase to catalyse oxidation of the lactic acid to pyruvic acid by NAD. Another system using steroid dehydrogenases and NAD can also be used to determine certain steroids. Another system which is suitable for glutamic acid determination uses glutamate dehydrogenase to catalyse oxidation of the glutamic acid to 2-oxoglutamic acid by NAD with the liberation of protons. An enzyme system suitable for the determination of glucose comprises glucose oxidase which catalyses oxidation of glucose to gluconic acid with the liberation of hydrogen peroxide. Another system of this type can be used to determine cholesterol using the enzyme cholesterol oxidase again with the liberation of hydrogen peroxide. Certain amines and amino acids can be similarly detected using the appropriate amine or amino acid oxidase. In addition other analytes may be detected through the use of enzymes linked to antibodies to said analytes so that binding of the analyte with the antibody converts the enzyme from a catalytically inactive form to a catalytically active form which can then catalyse release of protons or hydrogen peroxide by a suitable reactant. Thus for example analytes such as cytotoxic drugs e.g. ethotrexate; food toxins e.g. aflatoxins which are produced by moulds growing on peanuts, maize and wheat; and industrial effluents and toxic products, e.g. dioxin, may be determined using devices of the invention. Conveniently there may be used for example a system in which a suitable enzyme which catalyzes release of protons or hydrogen peroxide by suitable reagents, is conjugated to a sample of the desired analyte, by means of suitable protein modifying reactions e.g. using a carbodiimide to produce linking of carboxyl and amino groups, using reductive amination of aldehydes using sodiumcyanoborohydride and an amine; using acylation of amino groups with anhydrides; or any other suitable procedure known in the art. In the device ready for use the analyte-enzyme conjugate is bound by an antibody to the analyte. Thus .when the device is contacted with a test solution containing analyte molecules, these bind the antibody displacing the previously bound enzyme-analyte conjugate freeing it to catalyze reaction of the proton or hydrogen peroxide releasing reagent. In one example that may be mentioned there could be usedglucose oxidase enzyme with glucose reagent which releases hydrogen peroxide upon the glucose oxidase enzyme catalysed oxidation of glucose to gluconic acid.
As indicated above the enzyme support element is advantageously coated with a filter means for screening said enzyme support element and the polymer element to a greater or lesser extent from other materials present in the liquid sample to be tested which could interact with one or more of the enzyme, the enzyme catalysed reaction, and the polymer element. This is particularly desirable where the liquid sample is a biological fluid such as urine or a blood fraction which contains a whole variety of different substances. In general the filter means used will be substantailly impermeable to proteinaceous material and/or macromolecular substances. Suitable filter means include highly crosslinked polymeric water- swellable gels such as polyacrylamide and polysaccharose gels.
The filter means is conveniently in the form of a layer secured to the outer face of the conducting polymer film for example by polymerisation thereon in the case of a polymeric gel or by mechanical securing with the aid of external mechanical supports or restraints. Thus for example, the device may conveniently be mounted in a housing of an inert and impermeable electrically insulating material e.g. a plastics material such as polyvinylchloride, with a 'window' opening across a central area of the outer face of the filter means. In use of the deivce of the invention an unknown solution believed to contain the analyte is contacted with the second face of the enzyme support element either directly or through a filter means as defined hereinabove and the change in conductivity between the electrical connection means measured by connection thereto of a resistance measuring means. Thus in a further aspect the present invention provides a method of detecting a predetermined analyte in a liquid sample comprising the steps of contacting the liquid sample with the second face of the enzyme support element of the device of the invention either directly or through a filter means, selectively permeable to the analyte, and measuring the change in resistance between the connection means of the polymer element of said device.
Further preferred features and advantages of the invention will appear from the following detailed description given by way of example of a preferred embodiment illustrated with reference to the accompanying drawing in which : Fig. 1 is a generally schematic sectional elevation of a device of the invention in use in measuring the ethanol content of a liquid sample L.
Fig. 1 shows a device of the invention comprising a vessel 1 of an inert electrically insulating material such as glass having an electrically conducting polypyrrole layer 2 in the bottom 3 thereof. An ethanol permeable substantially electrically non-conducting enzyme support layer 4 is disposed on top of said polypyrrole layer 2 with a first face 5 in contact with the latter and a second face 6 covered in turn by a filter means layer 7. Two spaced apart electrical connections in the form of platinum wires 9 extend through the bottom wall 10 of the vessel 1 into the polypyrrole layer 2 and are connected 12 at their distal ends 13 to an ohm meter_ £_. The enzyme support layer comprises a highly cross- linked polymeric water-swellable gel such as a polyacrylamide or polysaccharose gel to which is secured the enzyme(s) to be used together with any necessary cofactors.. In the case of the device illustrated there is first formed a prepolymer of polyacrylamide having a molecular weight in the range from 1000 to 2000 to which is added ethanol dehydrogenase, and the co-enzymes NAD. The prepolymer is then cross-linked in conventional manner to entrap the enzyme and co-enzyme.
In order to convert the resistance measurements obtained from the ohm meter___f _ , a data processing unit D is connected thereto. This unit is adapted to record differences in resistance measurements between successive readings and process these in accordancewith previously established relationships obtainedusing known solutions to provide an output signal corresponding to the ethanol concentration present which is then displayed on a suitable visual display unit E>. EXAMPLE 1 - Construction of Ethanol Sensor Polypyrrole Film (2.5 x 1.1 cms. 0.2mm thick) was mounted on a glass slide support using two metal conductor legs secured to the film in spaced apart relation, with the aidof a suitable non-conducting resin adhesive such as that available under the Trade Name "Araldite" from the Ciba-Geigy Company of Basel Switzerland. This resin was also used to provide an insulating coating for the legs between the slide and the film. Suitable conductor leads for attachment to a conductivity orohm meter were connected to the metal conductor legs on the slide. The film element was then placed in a vessel to which was added activated polyacrylamide prepolymer (PAN)
(1.5g containing approximately 1000 u mol active esters) prepared in accordance with the procedures of Whitesides (A.Pollak et al J. Chem. Soc. 1980 Vol. 102 p.6324) dissolved in a buffer solution comprising 0.3 M Hepes buffer pH 7.5, 30 mM magnesium chloride and 0.3 mM NAD - ll -
tδ ml) during 2-3 min. Dithiothreitol (0.1 ml) was added followed by triethylenetetraamine (0.85 ml) to initiate cross-linking. After 2.5 minutes a solution of horse liver alcohol dehydrogenase (40 mg) in the above buffer (1 ml) was added. The polymer began to gel 2 minutes later and the polypyrrole film coated with the enzyme system - containing polyacrylamide gel was withdrawn. The coated film was then allowed to dry in air at room temperature for 1 hour and was then washed by immersion successively in solutions of the above buffer containing ammonium sulphate (50 mM) for 20 minutes and finally in buffer solution alone. The washed coated polymer film was allowed to dry overnight after which the sensor was ready for use. EXAMPLE II - Preparation of Glucose Sensor
The above described procedure for preparation of an ethanol sensor was repeated with a separate sample of polypyrrole film except that glucose oxidase (10 mg) was added in place of the horse liver alcohol dehydrogenase, and nicotinamide adenine and dinucloetide (NAD)was omitted from the buffer solution.
EXAMPLE III - Detection of ethanol
The Ethanol Sensor of Example I was first deprotonated by immersion in aqueous sodium hydroxide (1M) for 5 minutes. (If desired lower concentrations e.g. 0.5M can be used provided the immersion time is extended appropriately - to 30 minutes in this case.)
The Ethanol Sensor was then equilibrated by immersion in deionised water, removed from the water, superficial water shaken off, and the conductivity of the sensor then determined using a Solartron Schlumberger 1186 Electrochemical interface (available from the Solartron Limited of Farnborough, Hampshire, England). Ethanol (100 μl) was added to deionised water to give an ethanol concentration of 10 mM and the sensor immersed in the solution. The procedure formeasuring conductivity was repeated after successfive periods of 2 minutes immersion. Results
After 10 minutes, the current had risen by 0.9 mA and reached a maximum of 2.0 mA after 30 minutes. A further sample of ethanol (100 μl) was added to give a solution concentration of 20 mM and the experiment repeated. The current increase was 0.9 mA after 10 minutes and 2.8 mA after 30 minutes. A further sample of ethanol (100 μl) was added to give a solution concentration of 30 mM and the experiment repeated. The current increase was 1.2 mA after 10 minutes and 2.8 mA after 30 minutes. The initial deprotonation step described is in fact optional but does have the advantage of significantly increasing the sensitivity and responsiveness of the sensor. It is also possible to use a polypyrrole film in the sensor which film is in a substantially deprotonated form ab initio as a result of production thereof by electrochemical polymerisation at an overvoltage - preferably from 4.5 to 3.0V relative to SCE. EXAMPLE IV - Detection of glucose
The glucose Sensor was equilibrated by immersion in deionised water, the superficial water shaken off, and the conductivity determined as described in Example III. Glucose (100 mg) was added to give a solution concentration of 30 mM and the sensor immersed in the solution. The procedure for determining conductivity was repeated after successive periods of 2 minutes immersion. Results After 4 minutes, the current increase was 30 mA and reached a maximumof40 mA in 20 minutes. Following the same procedures but using two slightly thinner films prepared independently under substantially identical conditions a test solution containing 25mM glucose yielded current increases after 20 minutes of 37ma and 40 a .
EXAMPLE V - Preparation of cholesterol sensor The procedure in Example I for the preparation of an ethanol sensor was followed except that cholesterol oxidase (1 mg, Sigma Chemical Co. Ltd., Poole, England) replaced alcohol dehydrogenase and nicotinamide adenine dinucleotide. The gelling time was 2% in and cross- linking time was 2 minutes. EXAMPLE VI - Detection of cholesterol The cholesterol sensor was equilibrated as in Example III for the detection of ethanol. Its response to solutions of cholesterol water-containing 10% Brij 30 (a non-ionic polyethyleneoxide detergent available from I.C.I, pic of England)was determined. Results
On immersion in a solution of cholesterol (100 mM) the conductivity rose 3 mA in 15 minutes reaching a maximum of 6 mA in 70 minutes.

Claims

1. A device for use in the detection, in a liquid sample, of a predetermined analyte which is reactive under predetermined enzyme catalysed conditions so as to produce at least one of a proton and hydrogen peroxide, which device comprises an electrically conducting polymer element (2) having spaced apart connection means (9) for connection of said polymer element (2) , in use of the device, to an electrical circuit means (12) for directly or indirectly detecting changes in electrical resistance in said element (2) , said polymer containing conjugatable monomer units and being permeable to protons and where said analyte under said enzyme catalyzed conditions produces hydrogen peroxide, to hydrogen peroxide and having an electrical conductivity which is variable according to the amount of protons or hydrogen peroxide in contact therewith, and an enzyme support element (4) containing at least one enzyme and any cofactor(s) required in said predetermined enzyme-catalysed conditions, in an analyte permeable substantially non-conducting medium and having a first face (5) in contact with said polymer element (2) and a second face (6) disposable, in use, directly or indirectly in contact with a said liquid sample.
2. A device as claimed in claim 1 which device includes a filter means (7) selectively permeable to the analyte which filter means (7) is disposed at said second face (6) for screening said enzyme support element (4) from at least one other component of said liquid sample in use of the device. 3. A device as claimed in claim 2 wherein said filter means is substantially impermeable to at least one of proteinaceous material and macromolecular substances. 4. A device as claimed in claim 2 or claim 3 wherein said filter means comprises a highly cross-linked polymeric water-swellable gel.
5. A device as claimed in any one of claims 1 to 4 wherein is used an enzyme catalyst system (4) which produces protons when in contact with a said analyte, wherein the polymer element (2) is used in a reduced form in order to increase the sensitivity of the device.
6. A device as claimed in any one of claims 1 to 5 which device is in the form of a multilayer thin film device made up of a thin film polymer element (2) coated on at least one side with the enzyme support element (4) .
7. A device as claimed in any one of claims 1 to 6 wherein the connection means (9) are in the form of highly conductive metal electrodes extending into the polymer element (2) .
8. A device as claimed in any one of claims 1 to 7 wherein the polymer element (2) comprises a polymer having a conductivity in the range of from 10"^ to lθ2 S cm"1. 9. device as claimed in any one of claims 1 to 8 wherein the enzyme support element (4) contains an analyte specific dehydrogenase which in use of the device catalyses oxidation of the analyte with liberation of protons. ιo. A device as claimed in any one of claims 1 to 8 wherein the enzyme support element (4) contains an analyte specific oxidase which in use of the device catalyses oxidation of the analyte with liberation of hydrogen peroxide. ιι. A device as claimed in any one of claims 1 to 10 wherein said polymer element (2) , enzyme support element (4) , and any filter means (7) are mounted in a vessel (1) formed and arranged for holding, in use, a body of test solution (L) in contact, directly or indirectly through the filter means (7) , with the second face (6) of the enzyme support element (4) .
12. A device as claimed in any one of claims 1 to 11 wherein said enzyme support element (4) contains at least one enzyme linked to an antibody to said analyte, so that said enzyme is converted from an inactive to an active form upon reaction of said analyte with said antibody in use of the device, and wherein said enzyme support element (4) further includes at least one reagent reactive in the presence of said enzyme in its active form so as to produce at least one of a proton and hydrogen peroxide.
13. A device as claimed in any one of claims 1 to 12 having a said electrical circuit means connected to said connection means.
14. A method of detecting a predetermined analyte in a liquid sample comprising the steps of contacting the liquid sample (L) with the second face (6) of the enzyme support element (4) of a device (1) according to claim 1, either directly or through a filter means (7) , selectively permeable to the analyte, and measuring the change in resistance between the connection means (9) of the polymer element (2) of said device (1).
PCT/GB1987/000192 1986-03-19 1987-03-19 Biochemical detector WO1987005624A1 (en)

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WO1991006625A1 (en) * 1989-10-30 1991-05-16 Fritz Pittner Biosensor and process for producing it
DE19646505A1 (en) * 1996-11-12 1998-05-14 Itt Ind Gmbh Deutsche Device for carrying out tests on cell samples and the like
US8921093B2 (en) 2006-07-24 2014-12-30 Biocer Entwicklungs Gmbh Arrangement for on-line measurements on cells

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GB8710472D0 (en) * 1987-05-01 1987-06-03 Cambridge Life Sciences Amperometric method
WO2004114450A1 (en) * 2003-06-24 2004-12-29 Nec Corporation Method for determining alcohol concentration, apparatus for determining alcohol concentration, and fuel cell system including such apparatus

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FR2228839A1 (en) * 1973-05-07 1974-12-06 Bactomatic Inc Microorganism analysis - by measuring change in electrical conductivity
FR2282114A1 (en) * 1974-08-14 1976-03-12 Ouest Sa Comptoir Scient Tec Enzymatic analysis - for chemical and biological substrates, by electrical conductivity differences
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WO1991006625A1 (en) * 1989-10-30 1991-05-16 Fritz Pittner Biosensor and process for producing it
DE19646505A1 (en) * 1996-11-12 1998-05-14 Itt Ind Gmbh Deutsche Device for carrying out tests on cell samples and the like
US6376233B1 (en) 1996-11-12 2002-04-23 Micronas Intermetall Gmbh Device for conducting research on cell specimens and similar materials
US8921093B2 (en) 2006-07-24 2014-12-30 Biocer Entwicklungs Gmbh Arrangement for on-line measurements on cells

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AU7161487A (en) 1987-10-09
JPH01500054A (en) 1989-01-12
CA1260538A (en) 1989-09-26
AU594142B2 (en) 1990-03-01
EP0263125A1 (en) 1988-04-13
GB8606824D0 (en) 1986-04-23

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